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Site-specific epitope tagging of G protein-coupled receptors by bioorthogonal modification of a genetically encoded unnatural amino acid

机译:通过对遗传编码的非天然氨基酸进行生物正交修饰,对G蛋白偶联受体进行位点特异性表位标记

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摘要

We developed a general strategy for labeling expressed membrane proteins with a peptide epitope tag and detecting the tagged proteins in native cellular membranes. First, we genetically encoded the unnatural amino acid p-azido-l-phenylalanine (azF) at various specific sites in a G protein-coupled receptor (GPCR), C-C chemokine receptor 5 (CCR5). The reactive azido moiety facilitates Staudinger ligation to a triarylphosphine-conjugated FLAG peptide. We then developed a whole-cell-based enzyme-linked immunosorbent assay approach to detect the modified azF-CCR5 using anti-FLAG mAb. We optimized conditions to achieve labeling and detection of low-abundance GPCRs in live cells. We also performed an accessibility screen to identify azF positions on CCR5 amenable to labeling. Finally, we demonstrate a preparative strategy for obtaining pure bioorthogonally modified GPCRs suitable for single-molecule detection fluorescence experiments. This peptide epitope tagging strategy, which employs genetic encoding and bioorthogonal labeling of azF in live cells, should be useful for studying biogenesis of polytopic membrane proteins and GPCR signaling mechanisms.
机译:我们开发了一种通用策略,用于用肽表位标签标记表达的膜蛋白并检测天然细胞膜中的标记蛋白。首先,我们在G蛋白偶联受体(GPCR),C-C趋化因子受体5(CCR5)的各个特定位点对非天然氨基酸对叠氮基-1-苯丙氨酸(azF)进行了遗传编码。反应性叠氮基部分促进施陶丁格与三芳基膦缀合的FLAG肽的连接。然后,我们开发了一种基于全细胞的酶联免疫吸附测定方法,以使用抗FLAG mAb检测修饰的azF-CCR5。我们优化了条件,以实现活细胞中低丰度GPCR的标记和检测。我们还执行了可访问性屏幕,以识别CCR5上适合标​​签的azF位置。最后,我们展示了一种制备策略,用于获得适用于单分子检测荧光实验的纯生物正交修饰的GPCR。这种肽表位标记策略在活细胞中采用了azF的遗传编码和生物正交标记,对于研究多聚膜蛋白的生物发生和GPCR信号传导机制应该是有用的。

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